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Inactivation of stable viruses in cell culture facilities by peracetic acid fogging

机译:通过过乙酸雾灭活细胞培养设施中的稳定病毒

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Looking for a robust and simple method to replace formaldehyde fumigation for the disinfection of virus-handling laboratories and facilities, we tested peracetic acid fogging as a method to inactivate stable viruses under practical conditions. Peracetic acid/hydrogen peroxide (5.8%/27.5%, 2.0 mL/m 3) was diluted in sufficient water to achieve ≥ 70% relative humidity and was vaporized as 10 μm droplets in a fully equipped 95 m 3 laboratory unit. High titers of reovirus 3, MVM parvovirus and an avian polyomavirus were coated on frosted glass carriers and were exposed to the peracetic acid fog in various positions in the laboratory. After vaporization, a 60 min exposure time, and venting of the laboratory, no residual virus was detected on any of the carriers (detection limit 1 infectious unit/sample volume tested). The log reduction values were 9.0 for reovirus, 6.4 for MVM parvovirus, and 7.65 for the polyomavirus. After more than 10 disinfection runs within 12 months, no damage or functional impairment of electrical and electronic equipment was noted.
机译:为了寻找一种强大而简单的方法来代替甲醛熏蒸法来对病毒处理实验室和设施进行消毒,我们测试了过乙酸雾化法作为一种在实际条件下灭活稳定病毒的方法。将过氧乙酸/过氧化氢(5.8%/ 27.5%,2.0 mL / m 3)稀释到足够的水中以达到≥70%相对湿度,并在配备齐全的95 m 3实验室单元中以<10μm的液滴形式蒸发。将高滴度的呼肠孤病毒3,MVM细小病毒和禽多瘤病毒涂在磨砂玻璃载体上,并在实验室中的各个位置暴露于过乙酸雾中。蒸发后,经过60分钟的暴露时间,经过实验室通风,在任何载体上均未检测到残留病毒(检出限<1感染单位/样本量)。呼肠孤病毒的对数减少值为9.0,MVM细小病毒为6.4,多瘤病毒为7.65。在12个月内进行10次以上的消毒后,未发现电气和电子设备损坏或功能受损。

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